Literature DB >> 18939966

Exhaustion of the chloroplast protein synthesis capacity by massive expression of a highly stable protein antibiotic.

Melanie Oey1, Marc Lohse, Bernd Kreikemeyer, Ralph Bock.   

Abstract

Plastids (chloroplasts) possess an enormous capacity to synthesize and accumulate foreign proteins. Here we have maximized chloroplast protein production by over-expressing a proteinaceous antibiotic against pathogenic group A and group B streptococci from the plastid genome. The antibiotic, a phage lytic protein, accumulated to enormously high levels (>70% of the plant's total soluble protein), and proved to be extremely stable in chloroplasts. This massive over-expression exhausted the protein synthesis capacity of the chloroplast such that the production of endogenous plastid-encoded proteins was severely compromised. Our data suggest that this is due to translational rather than transcriptional limitation of gene expression. We also show that the chloroplast-produced protein antibiotic efficiently kills the target bacteria. These unrivaled expression levels, together with the chloroplast's insensitivity to enzymes that degrade bacterial cell walls and the elimination of the need to remove bacterial endotoxins by costly purification procedures, indicate that this is an effective plant-based production platform for next-generation antibiotics, which are urgently required to keep pace with rapidly emerging bacterial resistance.

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Year:  2008        PMID: 18939966     DOI: 10.1111/j.1365-313X.2008.03702.x

Source DB:  PubMed          Journal:  Plant J        ISSN: 0960-7412            Impact factor:   6.417


  114 in total

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4.  Inducible gene expression from the plastid genome by a synthetic riboswitch.

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5.  Unsolved problems in plastid transformation.

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Review 7.  Bacteriophage endolysins as novel antimicrobials.

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8.  Expression of HPV-16 L1 capsomeres with glutathione-S-transferase as a fusion protein in tobacco plastids: an approach for a capsomere-based HPV vaccine.

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Journal:  Hum Vaccin Immunother       Date:  2014-11-19       Impact factor: 3.452

9.  Stable production of peptide antigens in transgenic tobacco chloroplasts by fusion to the p53 tetramerisation domain.

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10.  Comparison of effectiveness of 5'-regulatory sequences in transplastomic tobacco chloroplasts.

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Journal:  Transgenic Res       Date:  2016-08-26       Impact factor: 2.788

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